Dimorphism and virulence in fungi

Dimorphism and virulence in fungi Bruce S Klein1,2,3,4 and Brad Tebbets3 The signature feature of systemic dimorphic fungi – a family of six primary fungal pathogens of humans – is a temperatureinduced phase transition. These fungi grow as a mold in soil at ambient temperature and convert to yeast after infectious spores are inhaled into the lungs of a mammalian host. Seminal work 20 years ago established that a temperature-induced phase transition from mold to yeast is required for virulence. Several yeast-phase specific genes, identified one-by-one and studied by reverse genetics, have revealed mechanisms by which the phase transition promotes disease pathogenesis. Transcriptional profiling of microarrays built with genomic elements of Histoplasma capsulatum and ESTs of Paracoccidioides brasiliensis that represent partial genomes has identified 500 genes and 328 genes, respectively, that are differentially expressed upon the phase transition. The genomes of most of the dimorphic fungi are now in varying stages of being sequenced. The creation of additional microarrays and the application of new reverse genetic tools promise fresh insight into genes and mechanisms that regulate pathogenesis and morphogenesis. The use of insertional mutagenesis by Agrobacterium has uncovered a hybrid histidine kinase that regulates dimorphism and pathogenicity in Blastomyces dermatitidis and H. capsulatum. Two-component signaling appears to be a common strategy for model and pathogenic fungi to sense and respond to environmental stresses. Addresses 1 Department of Pediatrics, University of Wisconsin School of Medicine and Public Health, Madison, WI, USA 2 Department of Internal Medicine, University of Wisconsin School of Medicine and Public Health, Madison, WI, USA 3 Department of Medical Microbiology and Immunology, University of Wisconsin School of Medicine and Public Health, Madison, WI, USA 4 University of Wisconsin Comprehensive Cancer Center, University of Wisconsin School of Medicine and Public Health, Madison, WI, USA

Paracoccidioides brasiliensis, Sporothrix schenkii, and Penecillium marnefiii. These primary pathogens are capable of converting from a nonpathogenic mold in the soil to a pathogenic yeast (or spherule in C. immitis) after infectious spores are inhaled into the lungs of human or other mammalian hosts. These fungi collectively cause over a million new infections a year in the United States alone, and remain latent after prior infection in tens of millions of people worldwide, in whom they may reactivate if the host becomes immune-deficient [1–5].

The biological importance of phase transition in dimorphic fungi The morphologic conversion of the dimorphic fungi from mold to yeast is required for virulence. In experimental studies of H. capsulatum, the transition to the yeast form is required for the establishment of disease. Treatment of mycelia with the sulfhydryl inhibitor p-chloromercuriphenylsulfonic acid (PCMS) permanently and irreversibly prevents the transition to yeast at 37 8C. PCMS-treated H. capsulatum failed to cause illness in a mouse model of lethal experimental infection, and no fungal colonies were recoverable from spleens of the infected mice [6]. This evidence suggests that the conversion to yeast is necessary for virulence in H. capsulatum. Conversion to the yeast form may offer protection against killing by neutrophils, monocytes, and macrophages. Drutz and Frey [7] showed that B. dermatitidis yeast are too large to be ingested by polymorphonuclear neutrophils (PMNs), unlike the much smaller conidia. In addition, both PMNs and peripheral blood monocytes are more efficient at killing conidia than yeast.

Yeast phase specific factors and their role in virulence

Introduction

The phenotypic switch from an environmental mold morphotype to a pathogenic yeast morphotype results in a change not only in cell shape, but also in the composition of the cell wall, the presence of antigenic molecules, and the expression of virulence traits. In B. dermatitidis, the conversion from mold-to-yeast results in an increased cell wall content of a-(1,3)-glucan and a decreased b-(1,3)-glucan content [8]. In the pathogenic yeast forms of several of the dimorphic fungi, including B. dermatitidis, H. capsulatum and P. brasiliensis, the level of a-(1,3)-glucan in the cell wall correlates with the level of virulence [9]. Additionally, as cells adapt to changes in temperature, multiple changes occur in the lipid composition of the plasma membrane, which leads to remodeling and reorganization of the membrane [10].

The systemic dimorphic fungi represent a family of six phylogenetically related ascomycetes: Blastomyces dermatitidis, Coccidioides immitis, Histoplasma capsulatum,

The role of a-(1,3)-glucan in virulence of H. capsulatum was formally investigated in recent work. a-(1,3)-Glucan

Corresponding author: Klein, Bruce S ([email protected])

Current Opinion in Microbiology 2007, 10:314–319 This review comes from a themed issue on Fungi Edited by Jim Kronstad Available online 23rd August 2007 1369-5274/$ – see front matter # 2007 Elsevier Ltd. All rights reserved. DOI 10.1016/j.mib.2007.04.002

Current Opinion in Microbiology 2007, 10:314–319

www.sciencedirect.com

Dimorphism and virulence in fungi Klein and Tebbets 315

synthase (AGS1), the gene that encodes this cell wall polymer, was demonstrated to be essential in pathogenicity of the fungus [11]. Either targeted gene disruption or silencing of its expression by RNA interference significantly impaired the growth of the yeast in macrophages in vitro, and its ability to colonize the lungs of mice. In additional studies [12], the regulation of a-(1,3)glucan production was found to require the function of the AMY1 gene product, a novel protein with homology to the alpha-amylase family of glycosyl hydrolases, and UGP1, a UTP-glucose-1-phosphate uridylyltransferase that synthesizes UDP-glucose monomers. Loss of AMY1 function in turn attenuated the ability of H. capsulatum to grow in and kill macrophages and to colonize murine lungs. The exact mode by which a-(1,3)-glucan influences the pathogenesis of infections with dimorphic fungi remains poorly understood. However, recent work has shed new light on how it may influence host–pathogen interactions. Successful infection by fungal pathogens depends on the subversion of host immune mechanisms that detect conserved cell-wall components such as b-glucans, which are recognized by dectin-1 receptors on host phagocytes [13]. Dectin-1 mediates the inflammatory response to fungi and facilitates pathogen clearance [14]. a-(1,3)-Glucan in the outermost layer of the H. capsulatum yeast cell wall may contribute to pathogenesis by concealing immunostimulatory b-glucans from detection by host phagocytic cells. In a recent study, the production of the proinflammatory cytokine TNF-a by phagocytes was suppressed either by the presence of the a-(1,3)-glucan layer on yeast cells or by RNA interference based depletion of the host b-glucan receptor dectin-1. These findings may reveal an important mechanism by which H. capsulatum thwarts the host immune system. During conversion to the pathogenic form, the dimorphic fungi express other phase-specific products that have been shown to be essential in virulence (Table 1). In

B. dermatitidis, only the yeast phase expresses the immunoreactive 120 kDa protein antigen BAD1 (formerly named WI-1) [15,16]. BAD1 binds to chitin on the yeast cell wall, and about 4.7  106 molecules are estimated to be present on each individual yeast cell [17]. This surface molecule functions as an adhesin and essential virulence factor that binds the fungus to complement type 3 receptors and CD14 on macrophages and lung tissue [18,19]. BAD1 also alters the host’s immune response by downregulating production of the pro-inflammatory cytokine TNF-a in phagocytes and upregulating production of the anti-inflammatory cytokine TGF-b, aiding in the progression of a pulmonary infection [20]. Additionally, BAD1 contains 35 copies of a 25 amino acid tandem repeat, each harboring an EF-hand that binds calcium, which enables growth of yeast in a calcium poor environment [21]. Likewise, in H. capsulatum, only the pathogenic yeast phase expresses a released calcium-binding protein (CBP1), which is essential for growth in macrophages in vitro, and survival in the host and pathogenicity in vivo [22,23]. H. capsulatum yeast also produce Yps3, a cell walllocalized protein that is not produced by the mycelial phase [24]. Yps3 localizes to the cell surface via an epidermal growth factor (EGF)-like domain that fixes chitin fibrils [25]. RNA interference of Yps3 expression significantly impaired the growth of the fungus in lungs and spleen in a murine model of pulmonary infection, indicating that expression is required for virulence (Jon P. Woods, personal communication). The search for virulence determinants in other dimorphic fungi has lead to the identification of a parasitic phasespecific adhesin SOWgp in the spherule form of C. immitis that binds to host extracellular matrix proteins that is important for both pathogenesis and survival in the host [26]. In P. marneffei, a catalase peroxidase has been identified as a phase specific product that is expressed during transition to the yeast form at 37 8C [27]; its role in virulence has not been investigated.

Table 1 Partial list of phase-specific factors that have been investigated in dimorphic fungal pathogens Fungus Blastomyces dermatitidis

Gene BAD1

Expression phase

Function

Reference [20,21,47,48]

bys1

Yeast

Adhesion, phagocytosis, calcium binding, modulation of host response Unknown

Histoplasma capsulatum

CBP1 yps-3 yps 21:E-9 MS8

Yeast Yeast Yeast Mold

Calcium binding Unknown Unknown Unknown

[23] [24] [50] [51]

Coccidioides immitis

SOWgp

Spherule

Binds laminin and fibronectin

[26]

Mold

Dextranase

[52]

Yeast

Catalase-peroxidase

[27]

a

Sporothrix schenkii

–

Penicillium marneffei

cpeA

a

Yeast

[49]

Genetic locus not identified.

www.sciencedirect.com

Current Opinion in Microbiology 2007, 10:314–319

316 Fungi

Expression analysis of phase-specific genes in dimorphic fungi The studies above have identified, characterized and analyzed, one-by-one, a handful of individual phase specific factors in the systemic dimorphic fungi. Some of these are indispensable for pathogenicity. Undoubtedly there are many more that remain to be identified and analyzed. The genomes of several of the dimorphic fungi are in varying stages of being sequenced and completed and this information along with microarrays should provide new insight into the identity and function of phase regulated genes that contribute to pathogenicity. Pending these studies, initial transcriptional profiling has been done in H. capsulaum and P. brasiliensis that sheds new light on phase regulated genes. Hwang et al. [28] created a 10 000 element genomic shotgun microarray with genomic fragments that are estimated to represent one-third of the genome. On probing the array with cDNA from mold and yeast, they identified approximately 500 genes that are expressed at a significantly higher level (>fivefold) in one phase versus the other. Of these, 217 genes were upregulated in the yeast form, and 271 in the mold form. Among the yeast-specific genes, one was upregulated from 50-fold to 100-fold, and 20 from 20-fold to 50-fold. Conversely, three genes were upregulated in the mold from 50-fold to 100-fold. In the latter group, TYR1 was upregulated in mold versus yeast by nearly 120-fold. TYR1 is an ortholog of a tyrosinase gene (MelC2) from the bacterium Streptomyces griseus. MelC2 is needed to produce melanin. Under normal culture conditions, H. capsulatum mycelia produce melanin, whereas yeasts do not. TYR1 is believed to be a candidate for the regulation of melanin production and establishment or maintenance of H. capsulatum in the mycelial form. In addition to confirming the yeast-phase specific expression of CBP1 and yps-3 with the shotgun microarray analysis, Hwang et al. [28] identified several genes involved in sulfur metabolism that were upregulated in the yeast phase. This is of interest because classical studies have established that sulfur metabolism influences the morphological state of H. capsulatum and other dimorphic fungi [29]. For example, the addition of exogenous sulfhydryl reducing agents (dithiothreitol) to the media locks cells in the yeast form independent of temperature, whereas the addition of sulfhydryl oxidizing agents (PCMS) locks cells in the mycelial form independent of temperature [29]. In H. capsulatum, some strains exhibit a requirement for the presence of cystine or cysteine in the culture medium to grow in the yeast phase. Microarray analysis identified a yeast-specific cysteine dioxygenase gene that was expressed 11-fold higher in yeast than in mycelia. In addition, several yeastexpressed genes share sequence similarity to genes that are involved in sulfur metabolism in other organisms: choline sulfatase; ATP sulfurylase (the first enzyme in Current Opinion in Microbiology 2007, 10:314–319

the sulfate-assimilation arm of the methionine/cysteine biosynthetic pathway); glutamate-cysteine ligase, which affects glutathione and glutamate metabolism); and methionine permease, which can mediate both methionine and cysteine uptake in Saccharomyces cerevisiae [30]. Using a different approach, Felipe et al. [31] analyzed the transcriptional profiles of P. brasiliensis to identify mycelial and yeast specific transcripts. They took advantage of 6022 ESTs (an estimated 80% of the fungal genome) from P. brasiliensis and used cDNAs from each phase to probe micro-array membranes. They identified 328 genes that were differentially expressed during the phase transition; 58 in the mycelium and 270 in the yeast. These upregulated genes fell into multiple categories relating to the cell cycle, stress response, drug resistance, and signal transduction pathways to name a few. The role of yeast-phase and mold-phase specific genes in establishing and maintaining these distinct morphological forms in P. brasiliensis and H. capsulatum, and in disease pathogenesis remains to be investigated.

Regulation of dimorphism and virulence in fungi From the foregoing, it is well recognized that transition from the mold-to-yeast form is a signature feature of this class of agents, and is required for the expression of virulence genes and pathogenicity. A major question is the field has been: How do these fungi sense a change in temperature and regulate the phase transition. Nemecek et al. [32] recently uncovered a long-sought regulator that controls the switch from a non-pathogenic mold form to a pathogenic yeast form in dimorphic fungi. They found that a hybrid histidine kinase (DRK1) functions as a global regulator of dimorphism and virulence in B. dermatitidis and H. capsulatum. DRK1 is required for phase transition from mold to yeast, expression of virulence genes, and pathogenicity in vivo. Disruption of DRK1 locks B. dermatitidis in the mold form at temperatures (37 8C) that normally trigger phase transition to yeast. RNA silencing of DRK1 expression in B. dermatitidis results in impaired BAD1 expression, severe alterations in the cell wall, and reduction in transcription of a(1,3)-glucan synthase and the yeast-phase specific gene BYS1. In H. capsulatum, DRK1 also regulates expression of the yeast-phase specific genes CBP1, AGS1 and yps-3. A DRK1 homolog is present and highly conserved in C. immitis, but has not yet been studied functionally. Hence, the hybrid histidine kinase DRK1 functions as a sensor of environmental change in the dimorphic fungi; it dictates their adaptation to environment stress inside mammalian hosts and their ability to cause disease. Two-component signaling systems are widespread in prokaryotes where signal transduction occurs via phosphorelay reactions [33]. When stimulated, a sensor histidine kinase www.sciencedirect.com

Dimorphism and virulence in fungi Klein and Tebbets 317

autophosphorylates a histidine residue and transfers this phosphate to an aspartate residue on a response regulator resulting in activation. The active response regulator controls transcription to elicit a cellular response from the histidine kinase. Eukaryote signal transduction has been thought to rely mainly on serine, theonine and tyrosine kinases, but histidine kinase two-component systems have been identified in lower eukaryotes and plants [34]. These pathways have recently been implicated in environmental sensing and cell development in eukaryotes [35], including in the opportunistic fungal pathogen Candida albicans, where they regulate filamentation and virulence [36,37,38].

multiple fungal pathogens. As described above, Drk1 in B. dermatitidis and H. capsulatum regulates the mold to yeast phase transition [32]. Deletion of CHK1, SLN1, or NIK1 in C. albicans impairs the formation of hyphae [36]. OS-1 of N. crassa is required for normal hyphal development as well as conidiation [45]. Importantly, inactivation of SLN1 homologues in fungal pathogens also attenuates their virulence. The involvement of two-component signaling systems in fungal sensing, morphogenesis and virulence, and their absence in humans, makes inhibitors of Sln1 homologues or its pathway components attractive drug targets [46].

Conclusions The most well understood fungal two-component signaling system is the SLN1 pathway of S. cervisiae. Sln1, a membrane bound hybrid-histidine kinase, is regulated by hyperosmotic stress [35]. Under normal osmotic conditions, Sln1 is autophosphorylated and transfers this phosphate to the phosphotransferase Ypd1 [39]. Ypd1 shuttles the phosphate from Sln1 to a response regulator, Ssk1, repressing its activity. When yeasts are exposed to hyperosmotic stress, Sln1 is inactive resulting in an unphosphorylated, active Ssk1. The response regulator turns on the Hog1 mitogenactivated protein kinase (MAPK) pathway, which increases production of the osmolyte glycerol [40]. Homologues of the Sln1 pathway components have been identified in a variety of pathogenic fungi including C. albicans, Aspergillus fumigatus, Cryptococcus neoformans, B. dermatitidis, H. capsulatum, and C. immitis [32,36,38,41,42]. Two-component signaling systems in the pathogenic fungi have diverse regulons including cell wall biosynthesis, virulence factor expression, drug resistance, and morphogenesis [32,42]. Though signaling pathway components are often similar in fungi, system structures and mechanisms of activation may differ from species to species. The HOG pathway of C. neoformans is an example. Unlike the canonical HOG pathway of S. cerevisiae, C. neoformans Hog1 is phosphorylated under normal conditions and functions as a repressor. When C. neoformans is exposed to stress, Hog1 is unphosphorylated, resulting melanin and capsule synthesis [43]. Pathogenic fungi contain multiple two-component signaling pathways. S. cerevisiae contains only one sensor histidine kinase (Sln1) as compared to three in C. albicans and 11 in N. crassa [36,44]. Signaling pathways of multiple sensor kinases often overlap resulting in redundant responses to stimuli, which complicates their characterization. For example, the three sensor histidine kinases of C. albicans (Sln1, Chk1, and Nik1) have distinct and redundant responsibilities in morphogenesis, cell-wall biosynthesis, and virulence [36]. Though challenging to delineate, two-component signaling systems regulate dimorphism and virulence in www.sciencedirect.com

It has long been known that morphogenesis from an environmental mold form to a pathogenic yeast form is essential for virulence in a family of ascomyetes that comprise the systemic dimorphic fungi. This event is triggered by exposure to host conditions, particularly temperature, and leads to programs needed for adaptation to the host environment, including genes for survival and virulence. Over the years, some of these genes have been identified and studied, one-by-one, providing a glimpse of how they promote disease pathogenesis. New tools for genetically manipulating these fungi, the sequencing of their genomes, and microarray analyses have provided a much deeper understanding of the many genes and some of the regulators involved during this extreme makeover inside the host. The future promises exciting new developments and further understanding of the regulatory networks, the downstream targets, and the role of these host-specific genetic programs essential for survival and virulence in mammalian hosts.

Acknowledgements The authors are supported by funds from the NIH and USPHS.

References and recommended reading Papers of particular interest, published within the annual period of review, have been highlighted as:  of special interest  of outstanding interest 1.

Galgiani JN: Coccidioidomycosis: a regional disease of national importance. Rethinking approaches for control. Ann Intern Med 1999, 130:293-300.

2.

Ajello L: In Distribution of Histoplasma capsulatum in the United States. Edited by Ajello LCW, Furcolow MF. Springfield Ill: Charles C. Thomas Publishers; 1971.

3.

Wheat LJ, Connolly-Stringfield PA, Baker RL, Curfman MF, Eads ME, Israel KS, Norris SA, Webb DH, Zeckel ML: Disseminated histoplasmosis in the acquired immune deficiency syndrome: clinical findings, diagnosis and treatment, and review of the literature. Medicine (Baltimore) 1990, 69:361-374.

4.

Chiller TM, Galgiani JN, Stevens DA: Coccidioidomycosis. Infect Dis Clin North Am 2003, 17:41-57, viii.

5.

Klein BS, Vergeront JM, Davis JP: Epidemiologic aspects of blastomycosis, the enigmatic systemic mycosis. Semin Respir Infect 1986, 1:29-39. Current Opinion in Microbiology 2007, 10:314–319

318 Fungi

6.

Medoff G, Kobayashi GS, Painter A, Travis S: Morphogenesis and pathogenicity of Histoplasma capsulatum. Infect Immun 1987, 55:1355-1358.

7.

Drutz DJ, Frey CL: Intracellular and extracellular defenses of human phagocytes against Blastomyces dermatitidis conidia and yeasts. J Lab Clin Med 1985, 105:737-750.

8.

San-Blas G, San-Blas F: Molecular aspects of fungal dimorphism. Crit Rev Microbiol 1984, 11:101-127.

9.

Hogan LH, Klein BS: Altered expression of surface alpha-1, 3-glucan in genetically related strains of Blastomyces dermatitidis that differ in virulence. Infect Immun 1994, 62:3543-3546.

10. Maresca B, Kobayashi GS: Dimorphism in Histoplasma capsulatum and Blastomyces dermatitidis. Contrib Microbiol 2000, 5:201-216. 11. Rappleye CA, Engle JT, Goldman WE: RNA interference in  Histoplasma capsulatum demonstrates a role for alpha-(1,3)glucan in virulence. Mol Microbiol 2004, 53:153-165. This report formally establishes the requisite role of AGS1 (and a-1,3glucan) in pathogenicity of H. capsulatum. The work is rigorously done using powerful new genetic tools for manipulating the organism; both RNAi and gene disruption. 12. Marion CL, Rappleye CA, Engle JT, Goldman WE: An alpha-(1,4) amylase is essential for alpha-(1,3)-glucan production and virulence in Histoplasma capsulatum. Mol Microbiol 2006, 62:970-983. This report establishes an essential element in the pathway that regulates AGS1 and alpha-1,3-glucan production. The work is significant for deciphering an upstream element in this pathway, and utilizing a forward genetics approach involving Agrobacterium tumefaciens for insertional mutagenesis to do so. 13. Brown GD: Dectin-1: a signalling non-TLR pattern-recognition  receptor. Nat Rev Immunol 2006, 6:33-43. An outstanding overview of this significant and rapidly evolving field in innate immunity. 14. Taylor PR, Tsoni SV, Willment JA, Dennehy KM, Rosas M,  Findon H, Haynes K, Steele C, Botto M, Gordon S et al.: Dectin-1 is required for beta-glucan recognition and control of fungal infection. Nat Immunol 2007, 8:31-38. Report of a Dectin 1 knockout mouse and its use in analyzing the role of this receptor in resistance to fungal infection. The work is significant for establishing the requisite role of Dectin 1 in resistance to fungal infection with Candida albicans. 15. Rooney PJ, Sullivan TD, Klein BS: Selective expression of the virulence factor BAD1 upon morphogenesis to the pathogenic yeast form of Blastomyces dermatitidis: evidence for transcriptional regulation by a conserved mechanism. Mol Microbiol 2001, 39:875-889. 16. Rooney PJ, Klein BS: Sequence elements necessary for transcriptional activation of BAD1 in the yeast phase of Blastomyces dermatitidis. Eukaryot Cell 2004, 3:785-794. 17. Klein BS, Jones JM: Isolation, purification, and radiolabeling of a novel 120-kD surface protein on Blastomyces dermatitidis yeasts to detect antibody in infected patients. J Clin Invest 1990, 85:152-161. 18. Newman SL, Chaturvedi S, Klein BS: The WI-1 antigen of Blastomyces dermatitidis yeasts mediates binding to human macrophage CD11b/CD18 (CR3) and CD14. J Immunol 1995, 154:753-761. 19. Brandhorst TT, Wuthrich M, Finkel-Jimenez B, Warner T, Klein BS: Exploiting type 3 complement receptor for TNF-alpha suppression, immune evasion, and progressive pulmonary fungal infection. J Immunol 2004, 173:7444-7453. 20. Finkel-Jimenez B, Wuthrich M, Brandhorst T, Klein BS: The WI-1 adhesin blocks phagocyte TNF-alpha production, imparting pathogenicity on Blastomyces dermatitidis. J Immunol 2001, 166:2665-2673. 21. Brandhorst TT, Gauthier GM, Stein RA, Klein BS: Calcium binding  by the essential virulence factor BAD-1 of Blastomyces dermatitidis. J Biol Chem 2005, 280:42156-42163. Current Opinion in Microbiology 2007, 10:314–319

This report establishes that BAD1 is a calcium-binding protein. The work is significant for establishing a new function for this virulence factor, demonstrating the domains that are responsible, illustrating how calcium binding induces conformational change, and showing that binding of calcium is needed for survival of the fungus in calcium poor conditions. 22. Batanghari JW, Deepe GS Jr, Di Cera E, Goldman WE: Histoplasma acquisition of calcium and expression of CBP1 during intracellular parasitism. Mol Microbiol 1998, 27:531-539. 23. Sebghati TS, Engle JT, Goldman WE: Intracellular parasitism by Histoplasma capsulatum: fungal virulence and calcium dependence. Science 2000, 290:1368-1372. 24. Keath EJ, Painter AA, Kobayashi GS, Medoff G: Variable expression of a yeast-phase-specific gene in Histoplasma capsulatum strains differing in thermotolerance and virulence. Infect Immun 1989, 57:1384-1390. 25. Bohse ML, Woods JP: Surface localization of the Yps3p protein  of Histoplasma capsulatum. Eukaryot Cell 2005, 4:685-693. This paper reports that Yps3 binds to the surface of H. capsulatum by an intriguing mechanism involving binding via a C-terminal domain that fixes to surface chitin. This feature is similar to that of BAD1 in B. dermatitidis and suggests a shared mechanism in fungi for coating the surface with protein. 26. Hung CY, Yu JJ, Seshan KR, Reichard U, Cole GT: A parasitic phase-specific adhesin of Coccidioides immitis contributes to the virulence of this respiratory Fungal pathogen. Infect Immun 2002, 70:3443-3456. 27. Pongpom P, Cooper CR Jr, Vanittanakom N: Isolation and characterization of a catalase-peroxidase gene from the pathogenic fungus, Penicillium marneffei. Med Mycol 2005, 43:403-411. 28. Hwang L, Hocking-Murray D, Bahrami AK, Andersson M, Rine J,  Sil A: Identifying phase-specific genes in the fungal pathogen Histoplasma capsulatum using a genomic shotgun microarray. Mol Biol Cell 2003, 14:2314-2326. This paper reports the first microarray analysis in dimorphic fungi. It represents a landmark effort in the use of arrays to profile phase-specific genes in H. capsulatum, and in the identification of nearly 500 such genes. Many interesting genes specific to the mold or yeast phase came out of this analysis and are under study. 29. Maresca B, Kobayashi GS: Dimorphism in Histoplasma capsulatum: a model for the study of cell differentiation in pathogenic fungi. Microbiol Rev 1989, 53:186-209. 30. Kosugi A, Koizumi Y, Yanagida F, Udaka S: MUP1, high affinity methionine permease, is involved in cysteine uptake by Saccharomyces cerevisiae. Biosci Biotechnol Biochem 2001, 65:728-731. 31. Felipe MS, Andrade RV, Arraes FB, Nicola AM, Maranhao AQ,  Torres FA, Silva-Pereira I, Pocas-Fonseca MJ, Campos EG, Moraes LM et al.: Transcriptional profiles of the human pathogenic fungus Paracoccidioides brasiliensis in mycelium and yeast cells. J Biol Chem 2005, 280:24706-24714. This paper is the first report of array based profiling of genes expressed during the phase transition of mold-to-yeast in P. brasiliensis. This paper also identifies many phase-regulated genes that govern diverse programs in this pathogen. 32. Nemecek JC, Wuthrich M, Klein BS: Global control of  dimorphism and virulence in fungi. Science 2006, 312:583-588. This paper is the first report of a global regulator of dimorphism and virulence in dimorphic fungi. The regulator is a hybrid histidine kinase that may sense changes in the environment such as temperature and trigger a two-component signaling pathway. 33. Cashin P, Goldsack L, Hall D, O’Toole R: Contrasting signal transduction mechanisms in bacterial and eukaryotic gene transcription. FEMS Microbiol Lett 2006, 261:155-164. 34. Thomason P, Kay R: Eukaryotic signal transduction via histidine-aspartate phosphorelay. J Cell Sci 2000, 113(Pt 18):3150. 35. Saito H: Histidine phosphorylation and two-component signaling in eukaryotic cells. Chem Rev 2001, 101:2497-2509. 36. Yamada-Okabe T, Mio T, Ono N, Kashima Y, Matsui M, Arisawa M, Yamada-Okabe H: Roles of three histidine kinase genes in www.sciencedirect.com

Dimorphism and virulence in fungi Klein and Tebbets 319

hyphal development and virulence of the pathogenic fungus Candida albicans. J Bacteriol 1999, 181:7243-7247. 37. Alex LA, Korch C, Selitrennikoff CP, Simon MI: COS1, a two-component histidine kinase that is involved in hyphal development in the opportunistic pathogen Candida albicans. Proc Natl Acad Sci U S A 1998, 95:7069-7073. 38. Kruppa M, Calderone R: Two-component signal transduction in  human fungal pathogens. FEMS Yeast Res 2006, 6:149-159. An outstanding review of two component signaling in human fungal pathogens with an emphasis on Candida albicans. 39. Posas F, Wurgler-Murphy SM, Maeda T, Witten EA, Thai TC, Saito H: Yeast HOG1 MAP kinase cascade is regulated by a multistep phosphorelay mechanism in the SLN1-YPD1-SSK1 ‘two-component’ osmosensor. Cell 1996, 86:865-875. 40. Maeda T, Wurgler-Murphy SM, Saito H: A two-component system that regulates an osmosensing MAP kinase cascade in yeast. Nature 1994, 369:242-245. 41. Pott GB, Miller TK, Bartlett JA, Palas JS, Selitrennikoff CP: The isolation of FOS-1, a gene encoding a putative twocomponent histidine kinase from Aspergillus fumigatus. Fungal Genet Biol 2000, 31:55-67. 42. Bahn YS, Kojima K, Cox GM, Heitman J: A unique fungal  two-component system regulates stress responses, drug sensitivity, sexual development, and virulence of Cryptococcus neoformans. Mol Biol Cell 2006, 17:3122-3135. This paper demonstrates that the two-component kinases Tco1 and Tco2 regulate the unique HOG pathway of the human fungal pathogen Crypotoccus neoformans. 43. Bahn YS, Kojima K, Cox GM, Heitman J: Specialization of the  HOG pathway and its impact on differentiation and virulence of Cryptococcus neoformans. Mol Biol Cell 2005, 16:2285-2300. This paper contrasts a highly pathogenic strain of Crypotoccus neoformans with a less virulent strain. A unique mechanism of HOG activation and its role in virulence factor regulation are identified in the highly virulent Crypotoccus neoformans.

www.sciencedirect.com

44. Catlett NL, Yoder OC, Turgeon BG: Whole-genome analysis of two-component signal transduction genes in fungal pathogens. Eukaryot Cell 2003, 2:1151-1161. 45. Alex LA, Borkovich KA, Simon MI: Hyphal development in Neurospora crassa: involvement of a two-component histidine kinase. Proc Natl Acad Sci U S A 1996, 93:3416-3421. 46. Bahn YS, Xue C, Idnurm A, Rutherford JC, Heitman J,  Cardenas ME: Sensing the environment: lessons from fungi. Nat Rev Microbiol 2007, 5:57-69. An outstanding review of how various members of the fungal kingdom sense and respond to diverse environmental cues. 47. Brandhorst TT, Wuthrich M, Warner T, Klein B: Targeted gene disruption reveals an adhesin indispensable for pathogenicity of Blastomyces dermatitidis. J Exp Med 1999, 189:1207-1216. 48. Hogan LH, Josvai S, Klein BS: Genomic cloning, characterization, and functional analysis of the major surface adhesin WI-1 on Blastomyces dermatitidis yeasts. J Biol Chem 1995, 270:30725-30732. 49. Burg EF 3rd, Smith LH Jr: Cloning and characterization of bys1, a temperature-dependent cDNA specific to the yeast phase of the pathogenic dimorphic fungus Blastomyces dermatitidis. Infect Immun 1994, 62:2521-2528. 50. Abidi FE, Roh H, Keath EJ: Identification and characterization of a phase-specific, nuclear DNA binding protein from the dimorphic pathogenic fungus Histoplasma capsulatum. Infect Immun 1998, 66:3867-3873. 51. Tian X, Shearer G Jr: The mold-specific MS8 gene is required for normal hypha formation in the dimorphic pathogenic fungus Histoplasma capsulatum. Eukaryot Cell 2002, 1:249-256. 52. Arnold WN, Nguyen TB, Mann LC: Purification and characterization of a dextranase from Sporothrix schenckii. Arch Microbiol 1998, 170:91-98.

Current Opinion in Microbiology 2007, 10:314–319